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Phenotypic and fine genetic characterization of the D locus controlling fruitacidity in peach
BMC Plant Biology 2009, 9:59 doi:10.1186/1471-2229-9-59
Karima Boudehri (kboudehr@bordeaux.inra.fr)Abdelhafid Bendahmane (bendahm@evry.inra.fr)
Gaelle Cardinet (gaelle.cardinet@bordeaux.inra.fr)Christelle Troadec (troadec@evry.inra.fr)Annick Moing (moing@bordeaux.inra.fr)
Elisabeth Dirlewanger (dirlewan@bordeaux.inra.fr)
ISSN 1471-2229
Article type Research article
Submission date 17 November 2008
Acceptance date 15 May 2009
Publication date 15 May 2009
Article URL http://www.biomedcentral.com/1471-2229/9/59
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BMC Plant Biology
© 2009 Boudehri et al. , licensee BioMed Central Ltd.This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0),
which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
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Phenotypic and fine genetic characterization of the D
locus controlling fruit acidity in peach
Karima Boudehri1, Abdelhafid Bendahmane
2, Gaëlle Cardinet
1, Christelle
Troadec2, Annick Moing
3,4, Elisabeth Dirlewanger
1§
1INRA, UR0419, Unité de Recherches sur les Espèces Fruitières, Centre de Bordeaux,
BP 81, F-33140 Villenave d'Ornon, France
2INRA-CNRS, UMR1165 Unité de Recherche en Génomique Végétale (URGV), 2
rue Gaston Crémieux, F-91057 Evry, France
3INRA - UMR619 Fruit Biology, INRA, Université de Bordeaux 1, Université de
Bordeaux 2, BP 81, F-33140 Villenave d’Ornon, France
4Metabolome-Fluxome Pole, IFR103 BVI, BP 81, F-33140 Villenave d’Ornon,
France
§Corresponding author
Email addresses:
KB: kboudehr@bordeaux.inra.fr
AB: bendahm@evry.inra.fr
GC: gaelle.cardinet@bordeaux.inra.fr
CT: troadec@evry.inra.fr
AM: moing@bordeaux.inra.fr
ED: dirlewan@bordeaux.inra.fr
- 2 -
Abstract
Background
Acidity is an essential component of the organoleptic quality of fleshy fruits.
However, in these fruits, the physiological and molecular mechanisms that control
fruit acidity remain unclear. In peach the D locus controls fruit acidity; low-acidity is
determined by the dominant allele. Using a peach progeny of 208 F2 trees, the D locus
was mapped to the proximal end of linkage group 5 and co-localized with major
QTLs involved in the control of fruit pH, titratable acidity and organic acid
concentration and small QTLs for sugar concentration. To investigate the molecular
basis of fruit acidity in peach we initiated the map-based cloning of the D locus.
Results
In order to generate a high-resolution linkage map in the vicinity of the D locus, 1,024
AFLP primer combinations were screened using DNA of bulked acid and low-acid
segregants. We also screened a segregating population of 1,718 individuals for
chromosomal recombination events linked to the D locus and identified 308
individuals with recombination events close to D. Using these recombinant
individuals we delimited the D locus to a genetic interval of 0.4 cM. We also
constructed a peach BAC library of 52,000 clones with a mean insert size of 90 kb.
The screening of the BAC library with markers tightly linked to D locus indicated that
1 cM corresponds to 250 kb at the vicinity of the D locus.
Conclusions
In the present work we presented the first high-resolution genetic map of D locus in
peach. We also constructed a peach BAC library of approximately 15x genome
equivalent. This fine genetic and physical characterization of the D locus is the first
step towards the isolation of the gene(s) underlying fruit acidity in peach.
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Background Peach [Prunus persica (L.) Batsch] belongs to the Spiraeoideae subfamily of the
Rosaceae [1]. The Prunus genus is characterized by species producing drupes as fruit,
and contains a significant number of economically important fruit tree species such as
almond (Prunus dulcis (Mill.)), apricot (Prunus armeniaca L.), sweet cherry (Prunus
avium L.), sour cherry (Prunus cerasus L.) and plum (Prunus domestica L.).
Compared to other tree species, peach has a relative small diploid genome (290 Mb)
[2], and a short juvenile phase (two to three years). Therefore, peach is considered as
a model species for Rosaceae family and a physical map of its genome has been
initiated [3].
Among fruit producing rosaceous crops, peach is the second most important fruit crop
in Europe after apple and the third worldwide (FAOSTAT: http://faostat.fao.org/).
However, the consumption of peaches and nectarines is stagnant due to the low
quality of fruits that are harvested at an immature stage for storage and shipment
reasons [4]. One of the major objectives for peach breeders is to find the right
compromise between quality and immaturity at harvest [5]. The variation in fruit
quality at harvest involves a large number of interrelated factors [6] among which
organic acid and soluble sugar contents and composition are major determinants [7].
In ripe peach fruit, malic and citric acids are the predominant organic acids, while
quinic acid accumulates in lower amounts [8, 9]. Moreover, the major soluble sugars
are sucrose, fructose, glucose and sorbitol [9, 10]. Sucrose is the predominant soluble
sugar at maturity while sorbitol accumulates at very low levels.
In peach, the D locus (D is for ‘Doux’ meaning ‘sweet’ in French) was described as
dominant and controlling the ‘low-acid’ character of fruit [11, 12]. Based on previous
segregation analyses of an F2 population (JxF) obtained from a cross between
‘Ferjalou Jalousia®
’ low-acid variety and ‘Fantasia’ normally-acid variety, the D
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locus was mapped on linkage group 5 [13]. It is co-localized with major QTLs for pH,
titratable acidity (TA), organic acids concentration and with small QTLs for sugars
concentration [14]. Low-acid peach fruit is characterized by reduced contents of malic
and citric acids [9], which, however, cannot be explained just by the reduced
expression or activity of phosphoenolpyruvate carboxylase (PEPC) [15], a key
enzyme involved in malate synthesis. ‘Ferjalou Jalousia®
’ fruit has half the
concentration of malic acid and one-fifth that of citric acid of ‘Fantasia’ variety [9].
Using the candidate gene approach, 18 genes involved in organic acid synthesis,
degradation or vacuolar storage were studied [16, 17]. Expression analyses in fruit of
six selected candidate genes did not show a clear difference between the normally-
acid and low-acid varieties [17]. The genes showing a modification of their
expression in the low-acid fruit compared to the normally-acid fruit were the
tonoplastic proton pumps PRUpe;AtpvA1, PRUpe;Vp2, and to a lesser extent
PRUpe;Vp1. PRUpe;Vp1 and PRUpe;Vp2 at citric acid peak and maturity, and
PRUpe;AtpvA1 during cell division showed higher expression in the fruit of the low-
acid variety (‘Ferjalou Jalousia®
’). However, none of these candidate genes were
located on linkage group 5, excluding their direct role in the control of acid content by
the D locus [17]. More recently, in the European ISAFRUIT Integrated Project
(http://www.isafruit.org/Portal/index.php), several candidate genes involved in fruit
quality were selected and tested on the JxF F2 mapping population. However, none of
them was located in the region of the D locus (Dirlewanger E., manuscript in
preparation)
Low-acid varieties have already been described in apple [18], tomato [19], grape [20]
and several Citrus species [21]. In apple, a non-acid mutant from the ‘Usterapfel’
variety showed a content in malic acid ten times less than the normally-acid one [22].
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The high level of malic acid was reported to be controlled by the dominant Ma allele
[23] suggesting that Ma and D act at different physiological control points. A cDNA-
AFLP analysis, coupled with a bulk segregant analysis (BSA) was recently used to
screen genes differently expressed between low- and high-acid apple fruits [24]. The
authors reported the isolation of a cDNA whose expression could only be detected in
low-acid fruit at an early stage of fruit development. Nevertheless, this cDNA showed
no homology with any sequences in public databases. Moreover, the Ma and D loci
are not located on homologous chromosomes: Ma is located on linkage group 16 in
Malus [25], homologous to linkage group 1 in Prunus [26] and D is located on
linkage group 5 in Prunus which is homologous to linkage groups 6 and 14 in Malus
[27]. For Citrus, the low level of citric acid is controlled by a recessive gene named
acitric [28]. Fruit acidity in Citrus seems to be linked to the capacity to accumulate
citric acid into the vacuole. Low-acid varieties accumulate low amount of citric acid
probably because it is exported out from the vacuole [29, 30]. Two candidate genes
such as acid invertase and cytoplasmic isocitrate dehydrogenase were identified to be
differentially expressed between acid and low-acid Citrus [30]. Fruit acidity can also
be controlled by several chromosome regions as in tomato where several QTLs for
titratable acidity and pH were identified [31, 32] and several candidate genes were
proposed [33]. However, to date the mechanism(s) of the genetic control of fruit
acidity remains to be elucidated.
In order to identify genes of interest, candidate gene approach can be used when
assumptions can be made regarding the biological function of the gene [34]. This
approach was successfully undertaken for several fruit traits including anthocyanin
content for which the biosynthesis pathway and regulating genes were well known
[35] and cell wall degradation where implicated genes were identified in other species
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[36]. However, to isolate agronomically important and botanically relevant genes with
unknown function and where no clear hypothesis can be made, chromosome landing
seems the main strategy by which map-based or positional cloning could be applied
[37]. The complexity of organic acids metabolic pathways as well as the difficult
understanding of the regulation of their transporters and channels and related proton
pumps [38, 39] has hampered, so far, the identification of the gene(s) associated to the
D locus using a candidate gene approach. Thus, in order to understand the molecular
and physiological bases of this trait, a positional cloning strategy was initiated and a
fine map of the D locus has been constructed. To identify the gene(s) underlying
acidity control at the D locus, the first step was to construct a fine map of the D locus.
The aims of the present work were: (1) the characterization of the fruit acidity trait,
(2) the increase of the number of markers tightly linked to the D locus, (3) the
conversion of the nearest markers into Sequence Characterized Amplified Region
(SCAR) and Cleaved Amplified Polymorphic Sequence (CAPS) markers, (4) the
construction of a high-resolution genetic map of this locus and definition of the
position of the D locus with new recombinant individuals phenotyped, and (5) the
evaluation of the genetic distance/physical distance ratio around the D locus using a
BAC library.
Results
Fruit acidity characterization
Among the 208 individuals used for the genetic linkage map, only 151 trees
producing fruit were phenotyped for pH and titratable acidity and were classified into
three subgroups corresponding to the three genotypes: homozygous for ‘Ferjalou
Jalousia®
’ allele (JJ) and for ‘Fantasia’ allele (FF), and heterozygous (JF) at the
targeted locus (Fig. 1). A significant difference (Student’s t-test, P<0.01) was
- 7 -
observed for pH and TA for the comparisons of JJ and JF genotypes, FF and JF
genotypes, and JJ and FF genotypes (pH mean values for JJ=4.57, JF=4.36, FF=3.63;
TA mean values JJ=36.5, JF=48.2, FF=109.7 meq/l) suggesting that the D allele is
partially dominant. Homozygous JJ genotypes showed values higher than 4.12 for pH
and lower than 51.9 meq/l for TA. On the opposite, pH and TA values for
homozygous FF genotypes were respectively lower than 3.93 and higher than
65.6 meq/l. The pH of heterozygous JF genotypes ranged from 3.80 to 4.87 and TA
ranged from 28.1 to 90.0 meq/l. Thus, normally-acid phenotypes that correspond
exclusively to genotypes FF showed pH value lower than 3.8 and TA value higher
than 100 meq/l while low-acid phenotypes corresponding to genotypes JJ or JF
showed pH values higher than 4.0 and TA value lower than 60 meq/l. These results
indicate that individuals with intermediate acidity (pH values between 3.8 and 4.0 and
TA values between 60 and 100 meq/l) can be either homozygous dd or heterozygous
Dd at the D locus and therefore, they cannot be reliably classified into normally-acid
or low-acid phenotype.
Identification and mapping of AFLP markers linked to the D locus
Among the 1,024 primer combinations tested, 960 provided readable amplification
products. Thirty to 90 bands were observed on AFLP gels per primer combination
with a size range from 60 to 1,000 bp, but only 6.5% of the bands were polymorphic
between the ‘Ferjalou Jalousia®
’ and ‘Fantasia’ parents. Markers whose bands were
present in BD1 and BD2 bulks and absent from Bd1 and Bd2 bulks were potentially
linked to the D locus (Fig. 2). A total of 34 markers were identified as putatively
linked to the D locus (Table 1). Nineteen primer combinations each revealed only one
D-linked marker, six primer combinations produced two D-linked markers (pGC-
AGG, pCA-GCG, pTC-CAC, pCA-ACC, pCA-TCC and pAA-ACA) and one primer
- 8 -
combination revealed three D-linked markers (pGC-TCT). As expected, all 34 AFLP
markers were mapped on linkage group 5. AFLP markers close to the D locus (within
22 cM) were clearly polymorphic between bulks. AFLP markers mapped further away
(beyond 27 cM) were polymorphic markers between bulks but with a very faint band
for “d” bulks. Fourteen AFLP markers were located within the first 10 cM containing
the D locus.
Conversion of AFLP markers into SCAR and CAPS markers
Nine AFLP markers linked to the D locus were converted into simple codominant
PCR-based markers. Four of them were codominant markers and five were dominant
markers (Table 1). The codominant AFLP markers (pGC-AGG 4 3 0J - 450F , pAC-
AAC4 0 2 J -4 12 F and pGG-TAC2 1 5 J -221 F) were successfully converted into SCAR
markers (D-Scar0, D-Scar1 and D-Scar2) and were confirmed as codominant markers
(Table 2, Fig. 3). The codominant AFLP markers pTC-GTA2 18 F -2 19J revealed a
deletion of one nucleotide in ‘Fantasia’ compared to ‘Ferjalou Jalousia®
’. After
sequencing the two alleles, three single nucleotide polymorphisms (SNPs) were
detected; one of them was revealed after digestion with the restriction enzyme AccI
and directly observed on agarose gel. This codominant Cleaved Amplified
Polymorphism Sequence (CAPS) marker was named D-Scar3 (Fig. 3).
For the dominant AFLP markers, primers were designed from the sequences of
individuals carrying the D allele. They were then tested on ‘Ferjalou Jalousia®
’,
‘Fantasia’ and on the F1-JF:21 hybrid used to construct the F2 mapping progeny. The
comparison of the sequences obtained for the pTG-TGG4 7 0 J marker revealed a
deletion of six nucleotides in ‘Fantasia’ as compared to ‘Ferjalou Jalousia®
’ sequence.
This AFLP marker was then transformed into a codominant SCAR marker (D-Scar6)
(Fig. 3). For pTC-CTG4 7 0J , the sequencing of the two alleles revealed one SNP. The
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alleles can be discriminated by digesting the PCR products with MseI. This CAPS
marker was called D-Scar7 (Fig. 3). For the three dominant AFLP markers pGT-
TTG1 8 8 J , pCA-GCG1 4 9 F and pCA-GCG1 3 2 J , no polymorphism was detected.
The six polymorphic SCAR markers were subsequently used to genotype the 208
individuals of the genetic linkage map; it confirmed that their localization was the
same as AFLP markers (data not shown).
Furthermore, considering the total size of the obtained sequences (2,711 bp), this
analysis revealed seven SNPs. Based on these results the frequency of the SNPs at the
vicinity of the D locus was estimated to 2.6 SNPs per kb.
High resolution mapping of the D locus
The fine mapping of the D locus was performed in two steps using the six SCAR
markers described in the present study and three SSR markers MA026a, BPPCT041
and CPPCT040 already mapped to the proximal end of the linkage group 5 [13, 26].
The first step was to genotype the 1,718 individuals from the seven segregating
populations with three SCAR markers (D-Scar0, D-Scar2 and D-Scar6) and two SSR
markers (MA026a and BPPCT041) spanning a region of 10.2 cM around the D locus
(Fig. 4). A total of 308 individuals were found to have at least one recombination
event between the farthest markers, MA026a and BPPCT041. The second step was to
genotype the resulting 308 recombinant individuals with the three other SCAR
markers (D-Scar1, D-Scar3 and D-Scar7) and CPPCT040 which were located within
the spanned region. According to the recombination events between these nine
markers, it was possible to determine the precise marker order on linkage group 5
(Fig. 4).
For the 149 recombinant individuals which produced fruits in 2007 and 2008, TA
mean values varied from 15 to 167 meq/l and pH mean values ranged from 3.36 to
- 10 -
5.59 (Fig. 5). Among these recombinants, 110 individuals were classified as
producing low-acid fruit, 12 were identified as producing normally-acid fruit and 27
were considered as intermediate and were therefore, not classified. Among the
individuals producing low-acid fruit, only 40 individuals recombining from
heterozygous (Dd) to homozygous (dd) were informative. Then, only 52 recombinant
individuals with extreme values for pH (from 3.36 to 3.68 for individuals with
normally-acid fruit and from 4.20 to 5.55 for individuals with low-acid fruit) and TA
(from 104 to 167 meq/l for individuals with normally-acid fruit and from 17 to 56
meq/l for individuals with low-acid fruit) were used to identify the position of the D
locus. Among the 52 recombinant individuals so selected, 36 recombinant individuals
between CPPCT040 and BPPCT041 indicated that the D locus was located upper than
CPPCT040, while fourteen other individuals recombining between MA026a and D-
Scar7 proved that the D locus was not localized between MA026a and D-Scar1
(Table 3). Two phenotyped individuals recombining between D-Scar0 and CPPCT040
reduced the interval containing the D locus: S5848-228 showed that the D locus was
located upper than CPPCT040 while S6422-237 demonstrated that it was located
below D-Scar0 (Table 3). Therefore, it can be concluded that the D locus is localized
in a 0.4 cM interval between D-Scar0 and CPPCT040 (Fig. 4).
Evaluation of the physical / genetic distance ratio around the D locus using a new BAC library
The peach BAC library produced from F1-JF:21 DNA contained about 52,000 clones.
Based on the analyses of a subset of clones, the average insert size was estimated at
90 kb, ranging from 50 to 130 kb. According to these preliminary results the covering
of this BAC library was estimated at 15-16 x the peach haploid genome. D-Scar0 and
D-Scar7 were used to screen the BAC library and four positive clones were found
with D-Scar0 and 12 with D-Scar7. Three of the four positive clones with D-Scar0
- 11 -
were found to be also positive when screened with D-Scar7. The ratio between the
genetic and physical distances was estimated using markers defined from BACend
sequences of a positive clone common to both D-Scar0 and D-Scar7 (Table 4). A
distance of 0.6 cM was estimated between the two CAPS markers F109-15-06 and
R109-15-06 (Table 4) derived from the BACend sequences of one BAC containing an
insert of 150 kb. This results in 1 cM corresponding to 250 kb in the region of the D
locus.
Discussion We describe in this paper major steps towards the cloning of the gene(s) controlling
fruit acidity in peach, by phenotypic, genetic and physical characterization of the D
locus.
The low polymorphism observed between ‘Ferjalou Jalousia®
’ and ‘Fantasia’ using
AFLP markers was previously reported using RFLP and SSR markers [13] and was
likely the consequence of the very low genetic distance between these two parental
varieties [13]. Polymorphic markers would have been considerably increased by deep
sequencing methods of the AFLPs [40]. Using the classical AFLP method in
combination with bulk segregant analysis, 14 AFLP markers located within the 10 cM
region harbouring the D locus were identified and no marker was mapped to another
linkage group. These results confirmed that acidity trait in peach is not complex and
should be controlled by a major gene.
Sequence analysis of the AFLP markers selected for conversion into SCAR revealed,
at the vicinity of the D locus, an SNPs frequency 3.6 fold lower than the one reported
in the ‘Texas’ x ‘Earlygold’ (TxE) reference Prunus map derived from an almond x
peach interspecific cross (Illa E., personal communication).
- 12 -
To more accurately position the D locus, it was necessary to identify individuals of
the extended population that had recombination events tightly linked to the D locus.
The strategy followed in the present work involving two successive steps (firstly the
genotyping of 1,718 individuals with the D locus-flanking markers and secondly the
analysis of the recombinant individuals with additional tightly linked markers)
reduced considerably the number of individuals that needed to be genotyped and
phenotypically characterized. Fruit acidity is usually evaluated by pH or TA
measurements. In this work, the use of both pH and TA was essential for the
characterization of fruit acidity. In addition, the definition of thresholds based on the
analyses of individuals without recombination event in the MA026a-BPPCT041
interval allowed a precise characterization of the phenotype. Thus, the phenotyping of
the recombinant individuals with the pH and TA threshold strategy prevented
misclassification of intermediate individuals that can be either homozygous (dd) or
heterozygous (Dd) for the D locus.
The development of tightly linked markers and the phenotyping of recombinant
individuals allowed the precise localization of the D locus. As fruit acidity is a major
selection criterion, the D-linked markers could be used for marker assisted selection
which would allow early selection of trees with the desirable character.
To estimate the relationship between the genetic and the physical distance at the
vicinity of the D locus we anchored a BAC clone to the genetic map. Based on this
analysis the ratio was estimated to 250 kb/cM. At the peach evergrowing (evg) locus
the ratio was estimated to 10 to 35 kb/cM [41]. These ratios are smaller than the
estimated average ratio on the TxE Prunus reference map [42] which is 553 kb/cM
according to the genome size [2]. This is not surprising, as the physical/genetic
- 13 -
distance ratio is known to vary along chromosomes [43-45]. The identification of the
physical/genetic distance ratio in the vicinity of the D locus was important for
estimating the number of walks needed for cloning the D locus. The D locus was
localized in a 0.4 cM interval corresponding to a physical distance of 100 kb. Thus,
one or two walks with BAC clones with an insert size of 90 kb should be sufficient to
identify a BAC clone harbouring the D locus.
Sequenced BAC clones in peach [41, 46], plum, apricot [46] and pear [47] revealed a
gene density of 14 to 36 genes per 100 kb genomic sequence. Thus, in the 100 kb D
locus region 14 to 36 candidate genes are expected. To identify the D gene(s) among
these candidate genes, the aim will be to map accurately the recombination events
relative to the predicted genes. To facilitate this analysis, the PPJFH BAC library was
constructed from the F1-JF:21 hybrid between ‘Ferjalou Jalousia®
’ and ‘Fantasia’ to
identify one BAC clone for each allele. The two orthologous BAC clones will be
sequenced and annotated and genetically dissected. In further analyses, the natural
variability of the candidate genes will be explored within a peach germplasm
collection to associate the haplotype to the phenotypic variation. Functional studies
such as reverse genetics experiments should then provide further evidence for or
against their involvement in fruit acidity.
The complete sequencing of the BAC clones will provide candidate genes for the D
locus. These candidate genes may be structural genes implicated in metabolism or
transport in agreement with our existing knowledge of fruit physiology or genes with
novel structural or regulatory functions. Sequencing data will also provide
information about Prunus genome organization in this particular region, which may
- 14 -
be compared to homologous region in other Rosaceae species and even other fruit
species. Microsynteny analysis across Rosaceae species will provide insight into gene
order, orientation and structural rearrangements of this particular region and through
comparative genomics, may contribute to improve our knowledge on evolutionary
and diversification processes among this family as demonstrated for Oryza [48].
Conclusions In conclusion, the present work describes, for the first time, the fine mapping of a
locus involved in a fruit quality trait on perennial plants via the chromosome landing
approach. The development of tightly linked markers and the phenotyping of
recombinant individuals allowed the precise localization of the D locus in a 0.4 cM
interval corresponding to 100 kb. Using the constructed PPJFH BAC library with a
mean insert size of 90 kb, one or two walks should be sufficient to identify a BAC
clone harbouring the D locus. To our knowledge, only few fine genetic maps were
realized using a large number of trees and only for resistance genes [49, 50]. One of
the major limitations for this strategy is the generation of a large population requiring
an extended orchard maintained over several years. Our mapping population of 2,086
plants that segregates for many agronomic traits as well as the PPJFH BAC library
will permit the genetic dissection of, not only the D locus, but also other traits such as
Af (aborting fruit), S (flat/round fruit), G (peach/nectarine) and Ps (pollen sterility).
This mapping population could be also exploited in any future genome sequencing
project in peach where anchoring sequences or BAC contigs to the genetic map is a
crucial step.
- 15 -
Methods
Plant material
The genetic linkage map was based on the segregation analyses of a peach F2
progeny. This progeny includes 208 individuals obtained from the selfing of a single
F1 hybrid (F1-JF:21) issued from a cross between ‘Ferjalou Jalousia®
’ a low-acid fruit
variety and ‘Fantasia’ a normally-acid fruit variety. This population segregates for six
Mendelian traits (low-acid/normally-acid fruit D, peach/nectarine G, flat/round fruit S,
clingstone/freestone F, pollen sterility Ps, aborting fruit Af) [13] and for several
characters involved in fruit quality as soluble sugar and organic acid concentrations
[17]. Among the 208 individuals, 151 produced fruit at maturity while 57 produced
flat fruit that fell after two months of growth and were not used in this study
(Table 5).
For the fine mapping of the D locus, a total of 1,878 F2 additional individuals were
obtained from the selfing of seven different F1 genotypes (Table 5). Three F1
individuals were issued from the cross between ‘Ferjalou Jalousia®
’ and ‘Fantasia’
(F1-JF:21, F1-JF:28, F1-JF:104), two from the reverse cross (F1-FJ:47, F1-FJ:49), one
from a cross between ‘Fantasia’ and ‘Fercopale Platina®
’ (F1-FP:10) and one from the
reverse cross (F1-PF:77). ‘Ferjalou Jalousia®
’ is homozygous for the dominant allele
(DD), ‘Fantasia’ is homozygous for the recessive one (dd) and the seven F1 hybrids
are heterozygous (Dd) for the D locus. ‘Ferjalou Jalousia®
’ dominant allele is derived
from ‘Kiang-Si’ that originated from China. ‘Fercopale Platina®
’ and ‘Ferjalou
Jalousia®
’ shared the same common grandparents (‘Kiang-Si’ and ‘Independence’)
(Fig. 6), and both had the same dominant allele for the D locus and produced flat
peaches. According to a marker assisted selection for the Af gene that segregated in
the 1,878 F2 individuals, 1,510 individuals were identified to produce fruit at maturity
and were therefore genotyped. Among them, 1,084 individuals were planted in 2005
- 16 -
and 426 in 2006. The fine map was based on the genotyping of a total of 1,718 F2
individuals including the mapping population of 208 individuals and the 1,510 F2
additional individuals that should produce fruit at maturity (Table 5).
Fruit acidity phenotyping
The 151 F2 individuals of the mapping population producing fruit and recombinant
individuals among the F2 progenies were phenotyped in 2007 and 2008. Two harvests
separated by four days were performed for each individual. For each harvest, six
fruits/individual were collected at maturity stage. TA and pH analyses were measured
on fruit juice by using an equal volume of juice from each fruit as described
previously [14].
To avoid any misclassification of recombinant individuals, we decided to rely on the
analyses of homozygous and heterozygous individuals and to define thresholds in
order to distinguish individuals with low-acid fruit from those with normally-acid
fruit. Individuals, without recombination event, were selected on their genotype in the
MA026a-BPPCT041 interval. Student’s t-test was used to compare pH and TA mean
values between homozygous and heterozygous individuals.
DNA extraction
Genomic DNA was extracted from young expanded terminal leaves. Fifteen
milligrams of fresh weight were collected for each tree in 96 collection microtubes of
1.2 ml containing a tungsten carbide bead (3 mm diameter). They were ground in
liquid nitrogen by using a Mixer Mill MM 300 (Retsch, Haan, Germany) for 1 min
and 30 s and genomic DNA was extracted according to the method previously
described [51].
- 17 -
BSA-AFLP
For Amplified Fragment Length Polymorphism (AFLP) assay combined with BSA,
two low-acid (D/D or D/d) DNA bulks (BD1, BD2) and two normally-acid (d/d) DNA
bulks (Bd1, Bd2) were used to identify putative markers linked to the D locus [52].
Individuals were selected among the 208 F2 used for the genetic linkage map
according to juice pH and TA values measured in 2002 and 2003. Equal amounts of
DNA from eleven individuals from the JxF F2 mapping population were pooled to
construct each bulk.
The AFLP technique was performed following the protocol developed by [53] with
some modifications. Genomic DNA (250 ng) was digested with two restriction
enzymes PstI and MseI in a volume of 17.5 -n0"Vjg"hktuv"RET"cornkhkecvkqp"ycu"
performed with primers having no selective nucleotide and then the second PCR
amplification was carried out with primers having two selective nucleotides for PstI
and three for MseI. PCR products were mixed with an equal volume of loading buffer
(95% formamide, 0.05% xylene cyanol, 0.05% bromophenol blue, 10 mM EDTA, pH
8.0). The mixture was heated for 5 min at 95°C, and then quickly cooled on ice. Each
sample mixture was loaded on a 4.5% denaturing polyacrylamide gel and visualized
by the silver staining system as described by [54]. Sixteen PstI+2 primers and 64
MseI+3 primers were tested consisting in a total of 1,024 primer combinations.
Markers derived from PstI+2/MseI+3 primer combinations were named as pXX-YYY
(X for the selective PstI nucleotides and Y for the selective MseI nucleotides).
Subsequently, polymorphic AFLP primer combinations between bulks were used to
screen the 208 F2 individuals of the mapping population.
Conversion of AFLP markers into SCAR and CAPS markers
AFLP markers linked to the D locus were selected for conversion into PCR markers
for further easy use in large-scale screening of the 1,718 individuals and BAC library.
- 18 -
After silver staining, marker fragments of the parents and of two F2 individuals were
picked with a tip on the dried polyacrylamide gel [55]"cpf"fkuuqnxgf"kp"37"-n"
deionized water. PCR amplifications were performed"wukpi"3"-n"fknwvkqp"ykvj"vjg"
same conditions as the selective PCR for AFLP reaction but with primers without
selective nucleotides. The products were separated on 2.0% agarose gel, purified
using a MinElute® PCR Purification Kit (Qiagen) and then cloned into the pGEM-T
easy vector (Promega, Madison, WI, USA). Clones were sequenced by Cogenics
(Meylan, France) and specific primers were designed using Primer3 software (version
V.0.4.0) based on these sequences. Designed primers were then tested for PCR
amplification on low-acid individuals, normally-acid individuals and also on ‘Ferjalou
Jalousia®
’, ‘Fantasia’ and the F1 hybrid (F1-JF:21). Reaction mixtures (10 µl)
contained 0.2 µM of each primer, 200 µM of dNTP, 10 ng template DNA, 0.26 U of
Taq DNA polymerase (Sigma-Aldrich), 1x PCR buffer provided with the enzyme.
PCR reactions were carried out for 2 min at 94°C, followed by 38 cycles of 45 s at
94°C, 45 s at annealing temperature, 45 s at 72°C, with final elongation for 5 min at
72°C. Finally, the amplified fragments were tested for their polymorphism on a 2 to 3
% agarose gel or 4.5% polyacrylamide denaturing gel.
Segregation analysis and map construction
Each polymorphic marker was tested by a chi-square for goodness of fit to the
segregation ratios 1:2:1 expected for codominant markers and 3:1 expected for
dominant markers in a F2 population. The linkage map was constructed using the
MAPMAKER/EXP V3.0 software [56]. Markers were first divided into linkage
groups using a critical LOD score threshold of 5. The Kosambi function was used to
convert recombination units into genetic distances.
- 19 -
Fine mapping
The 1,510 additional individuals that would have fruit at maturity were used to
complete the mapping population to a total of 1,718 individuals segregating for the D
locus. These individuals were screened for five markers, two SSR markers and three
new SCAR markers, spanning a large region around the D locus: MA026a and
BPPCT041, previously mapped on JxF linkage map [13] and three AFLP markers
transformed into SCAR markers. Recombinant individuals detected in this region
were genotyped with three other AFLP markers transformed into SCAR markers and
CPPCT040 a SSR marker mapped on the top of the linkage group 5 of
‘Texas’ x ‘Earlygold’ linkage map [26]. The phenotype of the recombinant
individuals compared to the recombination point enabled the localization of the D
locus. Among the 308 recombinant individuals detected, 149 individuals producing
fruit in 2007 and 2008 were phenotyped for fruit pH and TA.
Bacterial Artificial Chromosome (BAC) library construction
The Prunus persica PPJFH BAC DNA library was realized at URGV (INRA, Evry)
and constructed as described previously [57]. Nuclei were isolated from 32 g of young
leaves frozen in liquid nitrogen from F1 hybrid DNA heterozygous for all the
mendelian characters segregating in the JxF cross. Restriction fragments were
subjected to a double size selection in a CHEF-DRIII apparatus (Bio-Rad) by pulse
field gel-electrophoresis (PFGE). The DNA from the agarose slices was electroeluted
and cloned into the pIndigoBAC-5 (Hind III Cloning-Ready) Vector (EPICENTRE®
Technologies) for ligation reactions. Competent E. coli DH10B cells (Invitrogen)
were transformed by electroporation and transformants were selected on LB-Xgal-
IPTG plates containing 12.5 µg/ml chloramphenicol. White colonies were picked
using a Genetix Q-Bot and stored in 384-well microtiter plates (Genetix) at &80°C.
The PPJFH BAC library was composed of 150 plates corresponding to 57,600 total
- 20 -
BAC clones. BAC clones from each plate were mixed into pools of 384 clones
(designated ‘plate pools’). The BAC clones from each plate pool were resuspended
into sterilized water and DNA extracted before PCR reactions. In the first step,
positive plates were identified by screening the plate pools then in the second step the
16 clones of each of the 24 columns of the positive 384-well plates were pooled
together and screened to identify the positive column. The third step consisted in
identifying the positive BAC clone by screening the 16 clones of each positive
column pool. PCR amplifications were carried out as described before for PCR
experiments. Extracted DNA from BAC clones was digested with NotI and the
digestion products were subjected to pulsed-field gel electrophoresis (PFGE) as
described previously [57]: 25 µl DNA from each clone was digested by NotI in a 30
µl reaction mix and loaded on PFGE. Insert size was estimated using the PFGE
lambda ladder (BioLabs, Frankfurt, Germany).
To associate a genetic distance to the physical distance obtained with the PFGE,
primers were designed using Primer3 software (version V.0.4.0) based on two
BACend sequences of a chosen positive BAC clone for two markers (D-Scar0 and D-
Scar7). The primers of two markers were tested for PCR amplification on ‘Ferjalou
Jalousia®
’ and ‘Fantasia’ to identify polymorphism between the parents. Reaction
mixtures and PCR conditions were done as described for SCAR markers and the
amplified fragments were then sequenced. Obtained markers were used to genotype
only individuals recombining between D-Scar1 and CPPCT040 framing D-Scar0 and
D-Scar7.
Authors' contributions KB carried out the molecular genetic studies, the sequence alignment and drafted the
manuscript. KB and AB conceived and designed the experiments for the BAC library.
- 21 -
GC participated to AFLP mapping. CT carried out the BAC library pooling and
extraction. KB, GC, AM and ED performed the phenotypic analysis. ED and GC
participated in the genetic studies. AB and ED conceived the study and participated in
its design. AB, AM and ED helped to draft the manuscript. All authors read and
approved the final manuscript.
Acknowledgements This work was partly funded by INRA, the Ministery of Foreign Affairs of Algeria
and the “Conseil Régional d'Aquitaine” (Convention # 20054380505). The authors
thank Dr R. Monet for generating the F1 parents of the populations, the technical team
of UREF (C. Renaud, G. Capdeville, Y. Tauzin, L. Fouilhaux and J. Joly) for
producing the hybrids, fruit harvesting and biochemical characterization, the
Experimental Unit of INRA located at “Domaine des Jarres” for growing the trees,
Xavier Giresse for technical support and comments on an earlier version, Patricia
Faivre-Rampant for her comments and Drs Michel Caboche and Frédéric Laigret for
being at the initiative of the project, their support and helpful comments on this paper.
The authors thank also the unknown reviewers for helping us to improve this
manuscript.
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Figures
Figure 1 - Frequency distribution of pH and titratable acidity of fruit juice
Mean values observed in 2007 are represented. Distribution of F2 individuals, having
fruit at maturity, used for the genetic linkage map. White, black and grey bars indicate
homozygous genotypes for ‘Fantasia’ allele, ‘Ferjalou Jalousia®
’ allele and
heterozygous, respectively.
- 27 -
Figure 2 - AFLP markers detecting polymorphisms between low-acid bulks and normally-acid bulks revealed on polyacrylamide gel
AFLP markers showing a band in low-acid bulks (BD1 and BD2) but not in normally-
acid (Bd1 and Bd2) bulks are surrounded with a continuous line. AFLP markers
showing a faint band in Bd1 and Bd2 bulks, not selected for genetic mapping, are
surrounded with a dotted line.
Figure 3 - F2 individuals screened with SCAR markers on agarose gel
(a) D-Scar0 on 3% agarose gel (b) D-Scar1 on 2% agarose (c) D-Scar3 digested with
AccI, on 2% agarose gel (d) D-Scar6 on 3% agarose gel (e) D-Scar7 digested with
MseI, on 3% agarose gel. Specific band for each allele is indicated (d for normally-
acid and D for low-acid).
Figure 4 - Fine genetic map of the D locus on the distal end of linkage group 5
SSR and SCAR markers are on the right and genetic distances are indicated on the left
from the top (cM) and based on the analyses of 1,718 F2 individuals. The grey part
corresponds to the position of the D locus.
Figure 5 - Biplot of pH and titratable acidity of fruit juice
Mean values observed in 2007 are represented. pH and TA biplot for F2 individuals
recombining between MA026a and BPPCT041, phenotyped among the 1,718 F2
individuals. Individuals not included in squares are considered as intermediate.
Figure 6 - Origin of ‘Ferjalou Jalousia®’, ‘Fantasia’ and ‘Fercopale Platina®’ peach varieties
The phenotype for the D locus is indicated for each variety. Varieties with [D]
phenotype produce low-acid fruit and varieties with [d] phenotype produce normally-
acid fruit.
- 28 -
Tables
Table 1 - AFLP markers mapped on linkage group 5 (LG5) based on 208 JxF F2 individuals
AFLP
markersize in bp*
Position on LG5
(cM from the top)
Selection for
conversion into SCAR
SCAR marker
pAC-AAC4 0 2 J - 4 1 2 F 0 Yes D-Scar1
pGG-TAC2 1 5 J - 2 2 1 F 0 Yes D-Scar2
pGC-AGG4 3 0 J - 4 5 0 F 0.7 Yes D-Scar0
pTC-CTG4 7 0 J 0.7 Yes D-Scar7
pGT-TTG1 8 8 J 0.7 Yes Monomorphic
pCA-GCG1 4 9 F 0.9 Yes Monomorphic
pTC-GTA2 1 8 F - 2 1 9 J 1.8 Yes D-Scar3
pCA-GCG1 3 2 J 3.3 Yes Monomorphic
pTC-CAC2 0 6 J 4.1 No
pTG-TGG4 7 0 J 4.9 Yes D-Scar6
pCA-GTA3 9 0 J 5.6 No
pCA-ACC1 6 8 J 9.1 No
pGC-TCT2 3 2 F 9.2 No
pGG-TGA3 8 0 J 10 No
pCC-AGT2 2 3 J 11.7 No
pTA-TCC4 7 0 J - 4 7 5 F 11.7 No
pCC-GAA2 0 2 J 12 No
pCT-CAT2 0 3 J 12.2 No
pAG-GTA2 0 2 J 12.4 No
pTA-GTG6 0 0 J 15.2 No
pGC-TCT3 8 0 J 16.2 No
pGC-TCT3 7 0 F 17.4 No
pGT-TCT5 5 0 J 21.8 No
pAT-TTC3 6 0 J 22 No
pTA-CTC3 1 7 J 22.2 No
pCA-TCC4 0 0 J 27 No
pTC-CAC3 5 0 F 30.2 No
pAA-ACA2 5 3 F - 2 5 5 J 39.8 No
pCA-GAC1 5 8 J 40.7 No
pCA-ACC2 5 4 J 46.6 No
pGC-AGG5 0 0 J 47.8 No
pCT-ATC2 2 0 J 63.6 No
pAA-ACA4 0 0 J 68 No
pCA-TCC3 7 0 J 78.1 No
* Allele sizes for both parents are indicated for codominant markers, while only allele size for one
parent is indicated for dominant markers. J ‘Ferjalou Jalousia®’, F ‘Fantasia’.
- 29 -
Table 2 - SCAR and CAPS markers developed from AFLP fragments linked to the D locus
AFLP
markersize in bp1
SCAR
marker
Primer
sequence (5’-3’)
Size1
(bp)
P2 Annealing
temp.
(°C)
Enzyme
pGC-AGG4 3 0 J - 4 5 0 F D-Scar0 F GTGCACAGCTATCTCCTTTC
R CTCATGGCAACAACATATTC
160 (J)
175 (F)
SSR 52 no
pAC-AAC4 0 2 J - 4 1 2 F
D-Scar1
F GGGATGTGGGTATGTCGTA
R ACAAGGAGGAAGCTCTGG
345 (J)
364 (F)
SSR 55
no
pGG-TAC2 1 5 J - 2 2 1 F
D-Scar2
F CCTTACGTCTACGACGACAAC
R TGAGTCCTGAGTAATACTGTTCATGTG
142 (J)
148 (F)
InDel 54
no
pTC-GTA2 1 8 F - 2 1 9 J
D-Scar3
F GTTGACATGAAACAAATGACATTG
R CAGTCGTTCTTGTAGTTCACATGC
180 (J,F)
SNP
52
AccI
pTG-TGG4 7 0 J
D-Scar6
F CATGGCCCCATCTTTTCAC
R GACCAGTTGCATCTCATTCATATTGG
92 (J)
98 (F)
InDel
55
no
pTC-CTG4 7 0 J D-Scar7 F CTGGTCATCTACCGTCTC
R TCCAACTCCAAGGCTTGC
334 (J,F) SNP
55 MseI
1 (J) ‘Ferjalou Jalousia®’, (F) ‘Fantasia’, 2 Polymorphism observed.
Table 3 - Genotypes and phenotypes of F2 recombinant individuals for nine markers framing the D locus
1 P: Phenotype, [d]: normally acid fruit, [D]: low acid fruit, 2 F: homozygous for the ‘Fantasia’ allele (dd), H:
heterozygous highlighted in bold (Dd), * Number of F2 individuals having the same phenotype and genotype
Individual P 1 Genotype2 (G)
MA026a D-Scar2 D-Scar1 D-Scar7 D-Scar0 CPPCT040 D-Scar3 D-Scar6 BPPCT041
No of F2*
S8220-1186 [D] H H H H H H H H F 15
S8220-1321 [d] F F F F F F F F H 3
S5848-350 [D] H H H H H H H F F 11
S8220-1090 [d] F F F F F F F H H 3
S5848-332 [D] H H H H H H F F F 2
S6422-022 [d] F F F F F F H H H 2
S5848-228 [D] H H H H H F F F F 1
S6422-237 [D] F F F F F H H H H 1
S8220-2037 [d] H H H F F F F F F 1
S8220-1188 [D] F F F H H H H H H 7
S6361-020 [d] H H F F F F F F F 2
S5848-147 [D] F F H H H H H H H 1
S6422-452 [d] H F F F F F F F F 1
S8220-1045 [D] F H H H H H H H H 2
- 30 -
Table 4 - Markers developed from BACend sequences of a positive BAC clone with both D-Scar0 and D-Scar7
BACend
marker
Primer sequence (5’-3’) Size*
(bp)
Polymorphism Annealing
temp. (°C)
Enzyme
F109-15-06 F GTAGGATGAACTCAAAGGTG
R GTTGGTAATGACACTGGCTA
570
(J,F)
SNP 52 Tsp509I
R109-15-06
F GTGGACTTCATCCCATCTAC
R GGTCCAGAAGATGATGCAC
540
(J,F)
SNP 54
HincII
* (J) ‘Ferjalou Jalousia®’, (F) ‘Fantasia’
Table 5 - Origin of F2 individuals used for map construction and fine mapping of the D locus
Cross F1 name F2 name Number of F2
individuals
F2 used for the construction of the genetic linkage map
‘Ferjalou Jalousia®’ x ‘Fantasia’ F1-JF:21 S8220 208 Producing fruits 151
F2 additional individuals produced for the fine mapping of the D locus
’Ferjalou Jalousia®’ x ’Fantasia’ F1-JF:21 S8220 418
F1-JF:28 S6184 113
F1-JF:104 S7133 182
‘Fantasia’ x ‘Ferjalou Jalousia®’ F1-FJ:47 S6422 451
F1-FJ:49 S6421 106
‘Fantasia’ x ‘Fercopale Platina®’ F1-FP:10 S5848 405
‘Fercopale Platina®’ x ‘Fantasia’ F1-PF:77 S6361 203
Total of the additional F2 individuals 1,878
Additional F2 that will have fruits according to MAS for the Af gene 1,510
Total of the F2 individuals used for fine mapping 1,718
0
2
4
6
8
10
12
14
16
18
20
3,3 3,4 3,5 3,6 3,7 3,8 3,9 4 4,1 4,2 4,3 4,4 4,5 4,6 4,7 4,8
pH
Nu
mb
er
of
ind
ivid
uals
0
5
10
15
20
25
30
35
40
45
20-30 40-50 60-70 80-90 100-110 120-130 140-150 160-170
Titratable Acidity (meq/l)
Nu
mb
er
of
ind
ivid
uals
3.3 3.4 3.5 3.6 3.7 3.8 3.9 4 4.1 4.2 4.3 4.4 4.5 4.6 4.7 4.8
Figure 1
GT TG TC TT TA GAA GAC TCT GAA GAC TCT CAG CAC GAC CTG TCG CTG CTC TCA TCC
BD1 BD2 Bd1 Bd2
Pst+2
Mse+3
Primer combinations
Bulks
Figure 2
D
D
D
d
d
d
D
d
d
D
a
c
b e
d
Figure 3
MA026a 0.0 D-Scar2 0.4 D-Scar1 1.0 D-Scar7 2.0 D-Scar0 2.1 CPPCT040 2.5 D-Scar3 3.3
D-Scar6 5.2
BPPCT041 10.2
CPDCT022 86.1 Figure 4
3,0
3,5
4,0
4,5
5,0
5,5
6,0
0 20 40 60 80 100 120 140 160 180
Titratable acidity (meq/l)
pH
6.0
5.5
5.0
4.5
4.0
3.5
3.0
F2 with low-acid fruit
F2 with normally-acid fruit
Figure 5
F1 : 4 F1 : 12
Fercopale Platina® [D]
Self polination
Fantasia [d]
Bud mutation Bud mutation
Kiang-Si x Independence [D]
Red King x ン"
Ferjalou Jalousia® [D]
Self polination
Gold King x (Red King x ン+
Le Grand
Figure 6
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